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Infection and Immunity, July 1999, p. 3367-3375, Vol. 67, No. 7
Departments of Oral
Biology,1
Periodontology,2 and
Microbiology,4 State University of New
York, Buffalo, New York 14214, and Veterans Administration
Medical Center, Buffalo, New York 14214-30923
Received 27 January 1999/Returned for modification 9 March
1999/Accepted 2 April 1999
Porphyromonas gingivalis is a gram-negative, obligate
anaerobe strongly associated with chronic adult periodontitis. A
previous study has demonstrated that this organism requires superoxide dismutase (SOD) for its modest aerotolerance. In this study, we have
constructed a mutant deficient in SOD activity by insertional inactivation as well as a sod::lacZ
reporter translational fusion construct to study the regulation of
expression of this gene. We have confirmed that SOD is essential for
tolerance to atmospheric oxygen but does not appear to be protective
against hydrogen peroxide or exogenously generated reactive oxygen
species. Furthermore, the sod mutant appeared to be no more
sensitive to killing by neutrophils than the parental strain 381. SOD
appears to be protective against oxygen-dependent DNA damage as
measured by increased mutation to rifampin resistance by the
sod mutant. Use of the
sod::lacZ construct confirmed that
SOD expression is maximal at mid-log phase and is influenced by oxygen,
temperature, and pH. However, expression does not appear to be
significantly affected by iron depletion, osmolarity, or nutrient
depletion. The transcription start site of the sod gene was
determined to be 315 bp upstream of the sod start codon and
to be within an upstream open reading frame. Our studies demonstrate
the essential role that SOD plays in aerotolerance of this organism as
well as the selective induction of this enzyme by environmental stimuli.
The gram-negative obligate anaerobe
Porphyromonas gingivalis is one of the organisms most
strongly associated with chronic adult periodontitis (59).
P. gingivalis expresses numerous potential virulence
factors, such as fimbriae, hemagglutinins, lipopolysaccharides, and
various bacterial enzymes and proteases which are capable of
hydrolyzing collagen, immunoglobulins, iron-binding proteins, and
complement factors (2). One enzyme that may contribute to
the virulence of this organism is superoxide dismutase (SOD). This
enzyme, along with catalase and peroxidase, belongs to a specific
cellular system that has evolved for cellular protection against
oxidative stress. Interestingly, a previous study was unable to detect
either catalase or peroxidase activity in P. gingivalis
(2).
SOD has been found in nearly all aerobic organisms studied, as well as
in numerous obligate anaerobes that can tolerate transient exposure to
oxygen (11, 28). It acts to scavenge molecular oxygen and
its univalent reductants, thereby protecting the cell from the harmful
effects of these reactive oxygen species (ROS). The absence of SOD
activity causes a variety of oxygen-dependent phenotypic defects in
Escherichia coli, including a high rate of spontaneous
mutagenesis, severe defects in amino acid biosynthesis, and structural
instability of the cell envelope (27). Interestingly, overexpression of the iron-containing SOD (FeSOD) in E. coli
leads to increased oxygen sensitivity (54).
Eubacteria and archaea typically contain cytosolic SODs that require
manganese or iron as a cofactor (MnSODs and FeSODs, respectively). MnSOD is also found in the mitochondria of eukaryotes. MnSODs and
FeSODs have very similar structures and presumably evolved from a
common ancestral gene, and both may be present in an organism, such as
those encoded by the sodA and sodB genes in
E. coli (28). The conserved and well-distributed
nature of sodA, sodB, and other genes involved in
the oxidative stress response suggests the importance of these genes to
the organisms. For instance, although Legionella pneumophila
expresses a periplasmic copper- or zinc-containing SOD (CuZnSOD)
(encoded by the sodC gene), the cytoplasmic FeSOD is
essential for viability under normal culture conditions
(51). Originally considered to be specific to eukaryotes,
the sodC gene has been identified in a dozen or so bacteria
to date (28). In P. gingivalis, the cytosolic SOD
is encoded by one gene, sod, and utilizes Fe or Mn for
activity (3). Two other members of the
Bacteroides genus and one representative each from the
Propionibacterium, Streptococcus, and
Methylomonas genera also share this property (39).
The antimicrobial activities of monocytes and polymorphonuclear
phagocytes (PMNs) have been broadly characterized as being either
oxygen-dependent or oxygen-independent systems. Oxygen-dependent systems include the production of ROS, mediated by the phagocyte oxidative burst, and the reactive nitrogen intermediate, nitric oxide
(49). ROS include superoxide
(O2 Another product of activated phagocytes, nitric oxide (NO), has been
shown to be cytostatic or cytotoxic for a variety of invading
microorganisms. Its proposed actions include the interference with
iron-dependent enzyme functions in bacteria and reaction with
superoxide to form peroxynitrite, which in turn decomposes to form the
highly reactive hydroxyl radical and nitrogen dioxide (22).
The biological significance of these reactions in humans remains to be
determined; however, the important role of this system in the mouse
model is clear (49).
In this study, we describe the utilization of an isogenic SOD-deficient
mutant (CAL1) and a reporter gene fusion construct (CAL2) to determine
the role of SOD in the periodontopathogen P. gingivalis. We
have confirmed previous findings that SOD is essential for
aerotolerance (43) and now report that the P. gingivalis enzyme appears to confer different levels of protection against various ROS. Furthermore, in vitro studies of this organism suggest that SOD may not be essential for resistance to killing by
neutrophils, supporting similar findings for other organisms (45).
Bacterial strains and plasmids.
E. coli strains
were maintained in Luria-Bertani broth and on Luria-Bertani agar plates
at 37°C with the appropriate antibiotics. P. gingivalis
381 was grown at 35°C anaerobically in a Bioblend mixture (5% carbon
dioxide, 10% hydrogen, and 85% nitrogen) (Cryogenic Supply, Buffalo,
N.Y.) on enriched tryptic soy agar (ETSA) plates (Difco Laboratories,
Detroit, Mich.) as previously described (60). Broth cultures
of P. gingivalis were maintained in enriched tryptic soy
broth (ETSB) under the same conditions as the plates. All chemicals
were obtained from Sigma (St. Louis, Mo.) unless stated otherwise.
Construction of an isogenic SOD-deficient mutant (CAL1).
Plasmid pCC19, containing the sod gene, was constructed in
our laboratory and described previously (11). A 2.3-kb
HindIII-PstI fragment containing the intact
sod gene and its flanking regions from P. gingivalis ATCC 53977 was initially inserted into pUC19. Plasmid
pVA2198, containing an ermF-ermAM cassette, was obtained from F. Macrina (Medical College of Virginia, Richmond) and has been
described previously (19). pCC19 and pVA2198 were maintained in E. coli JM109 in the presence of 50 µg of ampicillin
per ml and 300 µg of erythromycin per ml, respectively. The
EcoRI-BamHI fragment containing the
ermF-ermAM cassette was isolated from pVA2198 and inserted
into the EcoRI-BglII-cleaved sod gene
in pCC19, thereby displacing an internal fragment of the gene. This plasmid, pCC19Em, was linearized and then used to electroporate P. gingivalis 381 essentially as previously described
(19). Strain 381 was used for mutant construction, since
this strain is more highly transformable than strain 53977. The
transformants were spread onto ETSA plates containing erythromycin (5 µg/ml) and gentamicin (25 µg/ml), and the plates were incubated
anaerobically for 10 to 14 days. Antibiotic-resistant colonies were
selected for Southern blot and functional analyses. Loss of SOD
activity was confirmed by two different methods. Crude cell extracts
were prepared following French press disruption in the presence of protease inhibitors (1 mM leupeptin or protease inhibitor cocktail). A
xanthine-xanthine oxidase coupled spectrophotometric assay
(38) and a nondenaturing polyacrylamide activity gel
(8) were employed to measure SOD activities. For the latter,
the stacking gel (4.8% polyacrylamide) was adjusted to pH 8.3, and the
resolving gel (10% polyacrylamide) was adjusted to pH 9.0.
Construction of a P. gingivalis
sod::lacZ strain.
The translational
fusion vector pMC1871 (55) (Pharmacia Biotech, Piscataway,
N.J.) was digested with BamHI to yield a fragment containing
the promotorless lacZ gene. This fragment was inserted into
the BglII site within the sod gene to yield an
in-frame fusion construct, pCC19Z. The shuttle vector pKDCMZ (courtesy
of K. Nakayama, Kyushu University, Fukuoka, Japan) (43) was
digested with PstI and SmaI to allow for
insertion of a PstI-MscI fragment from pCC19Z containing the sod::lacZ fragment, to
yield pKDSODZ. pKDSODZ was utilized as a suicide vector along with the
mobilizing plasmid R751 (40) for conjugal transfer of the
sod::lacZ fusion construct. This was
accomplished by mixing 2 ml of a mid-log-phase culture of P. gingivalis 381 with 2 ml of a mid-log-phase culture of E. coli DH5 Southern blot analysis.
P. gingivalis chromosomal
DNA was isolated from late-log-phase broth cultures by using the
recommended protocol supplied with the Puregene DNA Isolation Kit
(Gentra, Minneapolis, Minn.). After digestion with selected restriction
enzymes, DNA was loaded at 2.5 µg/lane onto 0.7% agarose gels, and
electrophoresis was performed. Gel preparation, transfer onto
Hybond-N+ membranes (Amersham, Arlington Heights, Ill.),
probe labeling, hybridization, and detection with the enhanced
chemiluminescence (ECL) system were performed as recommended by the
supplier (Amersham).
Comparison of environmental stresses on sod
expression.
Growth of P. gingivalis cultures was
determined by turbidimetric measurements of OD600;
viability was measured by plating serial dilutions of cultures onto
ETSA plates and incubating them anaerobically for 10 to 14 days for
viable-cell counting. All of the experiments were conducted by adding
the indicated compounds to cultures in ETSB medium. Aeration was
achieved by gently vortexing broth cultures in 50-ml tubes and placing
them in a shaking incubator at 200 to 250 rpm. Various concentrations
of hemin (0 to 100 µg/ml) were tested, with and without the addition
of the ferrous iron chelator 2,2'-dipyridyl (DPD) (125 µM). Iron
limitation was achieved by successive passaging of cultures in ETSB
containing 10 µg of hemin per ml and 125 µM DPD by previously
described methods (6). Hydrogen peroxide (30%, wt/wt) was
added to achieve the indicated concentrations, and pyrogallol was used
to generate extracellular superoxide (36). All samples were
incubated in duplicate, and the experiments were repeated at least
three times.
Human PMN bactericidal assay.
The PMN bactericidal assay is
a modification of an established protocol (62). Thirty
milliliters of peripheral venous blood was obtained, after informed
consent was obtained from the single volunteer, using a 19-gauge needle
to avoid activation of neutrophils. Three milliliters of 1.5%
Na2EDTA-phosphate-buffered saline (PBS) was added to the
blood sample and centrifuged for 20 min at 1,000 × g at
room temperature, and the top two phases were discarded. Forty
milliliters of 2% gelatin in a 0.9% NaCl solution was added, gently
mixed, and then placed in a 37°C water bath for 45 min. The top phase
was collected and centrifuged for 10 min at 1,000 × g at
room temperature. The pellet was collected and resuspended in 9 ml of
cold distilled water for 30 s, and erythrocyte lysis was stopped
by the addition of 3 ml of cold 3.5% NaCl together with 0.5 ml of
incomplete PBS. The sample was centrifuged for 5 min at 1,000 × g at room temperature, the supernatant was aspirated, and
the pellet was resuspended with complete PBS to a concentration of
107 cells per ml. Wild-type or CAL1 (50 µl; 2 × 107 CFU) samples were added to mixtures containing
combinations of human agammaglobulinemic serum (5%, as a complement
source; from M. E. Wilson, UMDNJ-NJDS, Newark, N.J.), rat
anti-P. gingivalis 2561 (0 to 100 µg/ml; from R. J. Genco, SUNY at Buffalo, Buffalo, N.Y.), and 107 neutrophils
in complete PBS. The contents of each tube were mixed thoroughly
following bacterial addition, after which (time zero) 50 µl was
rapidly withdrawn and transferred to tubes containing 4.95 ml of
sterile H2O with 0.2% filter-sterilized bovine serum albumin. Following 1 min of incubation at room temperature with gentle
mixing, 50 µl of the PMN lysate was removed and transferred to
sterile tubes containing 1 ml of prereduced ETSB. Aliquots of 0.1 ml
(~250 to 300 CFU) were plated onto ETSA plates and immediately placed
in an anaerobic chamber. Following removal of time zero samples, the
polypropylene tubes containing samples were placed onto a rotator with
continuous end-over-end rotation at 8 rpm in a humidified
CO2 incubator at 37°C. Samples were withdrawn at 20, 40, and 60 min and processed identically to the time zero samples. Plates
were incubated anaerobically for 10 to 12 days, and colonies were counted.
Spontaneous mutations rates.
Mutagenesis, as measured by
development of rifampin resistance, was determined for wild-type 381 and mutant CAL1. Overnight cultures were used to inoculate prereduced
medium and allowed to grow to mid-log phase, as determined by
OD600 values. Cultures were then exposed to shaking aerobic
culture conditions at 37°C for 15 min and then placed in a GasPak
holding jar containing H2 and CO2 (BBL GasPak
Plus, Becton Dickinson, Cockeysville, Md.) until the cultures reached
mid-log phase. OD600 values were recorded, and serial
dilutions of respective cultures were performed, with subsequent
plating on ETSA plates containing gentamicin (25 µg/ml) for CFU
determination. Two hundred microliters of undiluted samples was plated
on ETSA plates containing gentamicin (25 µg/ml) and rifampin (1 µg/ml) and placed under anaerobic conditions as described above.
Mutation rates were calculated by dividing total rifampin-resistant CFU
by total CFU per ml of culture.
RNA isolation and Northern blots.
Total RNA was isolated
from P. gingivalis cells grown to mid-log phase by a
modification of a previous method (60). The MscI-BglII sod fragment was isolated
from pCC19, and 300 ng was used to probe the membranes by using the ECL
detection system as described previously (Amersham).
Transcription start site determination.
An 18-mer
oligonucleotide (SOD Construction of the SOD-deficient mutant (CAL1).
The
sod gene from P. gingivalis 53977 was previously
isolated and shown to be oriented between the prtT gene and
an uncharacterized open reading frame (ORF) (Fig.
1) (11). Insertional
inactivation of the strain 381 sod gene with an
Emr cassette was carried out as indicated in Fig.
2. We confirmed a double-crossover
recombination event by Southern blot hybridization with DNA probes
derived from fragments containing the sod gene of P. gingivalis 53977 and the Emr cassette (data not
shown). This event resulted in the deletion of an internal fragment of
the sod gene and the insertion of the Emr
cassette into the chromosome of P. gingivalis 381, producing a stable, insertionally inactivated mutant (CAL1) resistant to erythromycin (up to 25 µg/ml) (Fig. 1 and 2). In addition, the loss
of SOD activity was confirmed by using both a SOD activity gel and a
spectrophotometric method (data not shown). As has been previously
observed for this organism (43), deletion of the sod gene resulted in a profound loss of aerotolerance. In
the present study, a loss of viability of more than 4 orders of
magnitude within 1 h of aerobiosis was noted. Apart from
phenotypic changes that could be directly ascribed to loss of SOD
function, CAL1 appeared to maintain properties essentially similar to
those of the wild type. Differences were often seen in the form of a
prolonged lag phase, difficulty in recovery from stationary-phase
cultures, and decreased maximal OD in stationary phase.
0019-9567/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Role of Superoxide Dismutase Activity in the
Physiology of Porphyromonas gingivalis
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
·), hydrogen peroxide
(H2O2), singlet oxygen ('O2), and
hydroxyl radical ( · OH). Numerous microorganisms
counter these antimicrobial species by impairment of phagocytosis,
alterations of microbicidal activity, or attenuation of the oxidative
burst. Specifically, P. gingivalis proteolytic activity
inhibits the generation of ROS in PMNs, thus suppressing bactericidal
ability (44). In addition, purified SOD from P. gingivalis added exogenously partially protected the organism from
this method of killing by PMNs (4).
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
(containing pKDSODZ and R751) and with chloramphenicol (25 µg/ml) and tetracycline (10 µg/ml). The sample was centrifuged for 5 min at 3,000 × g at 4°C, resuspended in 0.2 ml
of ETSB, and plated onto ETSA plates. The plates were incubated for
2 h aerobically at 37°C and then transferred to an anaerobic
chamber for 36 h. Bacterial growth on plates was harvested with a
sterile cotton swab and resuspended in 1 ml of ETSB, and 0.2-ml
aliquots were spread onto ETSA plates containing gentamicin (100 µg/ml) and erythromycin (5 µg/ml) and grown anaerobically for 10 to
14 days at 35°C. Colonies were screened by Southern blot analysis for
preliminary confirmation of the correct construction.
-Galactosidase assays.
The -galactosidase assay was a
modification of a previously published protocol (41).
Cultures of P. gingivalis were harvested (1.5 ml) after
growth under the indicated conditions, the optical density at 600 nm
(OD600) was recorded, and the culture was centrifuged for 8 min at 16,000 × g at 4°C. The pellet was resuspended
in 0.9 ml of buffer Z (41) and 0.1 ml of toluene, vortexed
vigorously, and placed in a shaking incubator at 30°C for 45 min,
with vortexing every 15 min. Samples were then centrifuged for 8 min at
16,000 × g at 4°C, 250 µl was aspirated (including
the top organic phase), and 250 µl of ONPG
(o-nitrophenyl--D-galactoside) was added and vortexed vigorously. Samples were then placed at 30°C in a shaking incubator for 15 to 45 min, and then the reaction was stopped with 0.5 ml of 1 M Na2CO3 and the sample was centrifuged
for 8 min at 16,000 × g at 4°C (this obviated the
need for spectrophotometric measurement at 550 nm). One milliliter was
used for OD420 measurement, and calculations were performed
by using established formulae; enzyme activities were expressed in
Miller units (41). All assays were performed in duplicate or
triplicate and repeated at least three times.
; 5'-CGTGCCGATGATGAGCTT-3')
corresponding to a location approximately 110 nucleotides
downstream of the sod start codon was used as a primer. In
addition, a 17-mer oligonucleotide (UPSODR;
5'-GCTGTCATCAGTCACGT-3') and a 19-mer oligonucleotide
(UPSODR2; 5'-GGCTGTGGTACCTTGAAGA-3') corresponding to
positions approximately 100 and 40 nucleotides, respectively, downstream of a putative transcription start site were used as primers
and end labeled with [
-32P]ATP (DuPont, NEN Research
Products, Wilmington, Del.). Reverse transcriptase (Gibco BRL) was used
to extend these primers to produce cDNA complementary to P. gingivalis mRNA following annealing. After RNase A treatment, the
resulting end-labeled cDNA was electrophoresed on 5 and 8% Long
Ranger-urea gels (FMC BioProducts, Rockland, Maine). Dideoxy sequencing
reaction mixtures with pCC19 and the above-described primers and with
M13mp18 and the 
40 primer were also electrophoresed for reference.
Dried gels were exposed to Kodak X-Omat AR film, and the sod
transcription start site was determined by counting the bases from the
respective primers as described previously (56).
RESULTS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
View larger version (5K):
[in a new window]
FIG. 1.
Schematic of the P. gingivalis 53977 chromosome region containing the sod gene.
View larger version (22K):
[in a new window]
FIG. 2.
Plasmid maps for construction of the sod
mutant (CAL1).
Role of SOD in sensitivity to environmental stress. In virtually all organisms studied to date, SOD expression has been to shown to be affected by specific environmental conditions as well as the growth rate of the organisms. Therefore, to test the potential inability of CAL1 to tolerate selected environmental stress, we compared the growth and viability of the wild type and CAL1 in the presence of elevated temperatures, ROS, and human PMNs.
The loss of SOD activity had no effect on the ability of P. gingivalis to grow anaerobically at temperatures of up to 45°C, although both wild-type and CAL1 growth steadily declined after several hours at increased culture temperatures. Neither wild-type P. gingivalis nor CAL1 was able to survive at 50°C. Furthermore, these increased temperatures did not appear to contribute to an additional loss of viability under aerobic conditions for CAL1 compared to the wild type (data not shown). Hydrogen peroxide is a product of the SOD enzyme, is included in antimicrobial prophylaxis, and is produced by numerous oral species (50). Although it has been suggested that the peroxide and superoxide stress responses are distinct (17), it was of interest to determine if the sod mutant was more sensitive to H2O2. H2O2 at final concentrations of 1 µM to 100 mM was added to cultures, and the cultures were incubated anaerobically and aerobically. Both cultures were exquisitely sensitive to H2O2 concentrations of 1 mM and greater, resulting in a loss of viability of more than 7 orders of magnitude. As little as 25 µM H2O2 resulted in a decrease of growth and viability for both the wild type and the CAL1 mutant. Therefore, the sod mutant CAL1 is no more sensitive to H2O2 than the parental organism. Pyrogallol is a compound that upon degradation generates superoxide in the extracellular environment, and it has been suggested that this ROS cannot penetrate cellular membranes (33). These molecules may therefore have direct and local effects on cellular membranes or may produce a free radical cascade that may allow for more remote deleterious effects (42). The present results indicate that although both the wild type and CAL1 are sensitive to as little as 2 mM pyrogallol, CAL1 is no more sensitive than the wild type (data not shown). This suggests that the cytoplasmic FeMnSOD of P. gingivalis does not protect the organism from superoxide generated in the extracellular milieu. To assess the role that SOD may have in conferring protection against killing by phagocytes, we compared the survival of opsonized CAL1 versus opsonized wild-type P. gingivalis after coincubation with human neutrophils. Previous studies have differed on the protective role that SOD may play against professional phagocytes (12, 20). In our study, nonopsonized wild-type P. gingivalis preincubated with PMNs maintained approximately 50% viability after 20 min. Addition of human complement, anti-P. gingivalis antibody, or both increased killing; the addition of antibody led to increased killing in a dose-dependent fashion. This correlates with previous studies examining killing of P. gingivalis by PMNs (14, 15). After determination of appropriate assay conditions, there appeared to be no difference between the two genotypes, with approximately 90% killing after 20 min for both the wild type and the mutant CAL1 in the presence of PMNs, complement, and antibody. Incubation periods of 40 and 60 min did provide for limited additional killing; however, it appeared that the kinetics of killing in this system were rapid and efficient. Unfortunately, shorter incubation periods could not be studied consistently, due to the number of necessary controls and processing steps associated with each sample. These data, taken together with those from the pyrogallol experiments, suggest that cytoplasmic SOD does not appear to protect P. gingivalis against the antibacterial activity of human neutrophils. SOD has been demonstrated to be protective to DNA against oxidative damage that ultimately results in chromosomal mutations (16). Therefore, we examined and compared ROS-induced mutation rates in the wild type and CAL1 as demonstrated by resistance to rifampin, an antibiotic known to be effective against P. gingivalis. Our results demonstrated that CAL1 has, on average, an approximately 6.8-fold-higher spontaneous mutation rate than P. gingivalis 381. This strongly suggests the importance of the cytoplasmic sod gene in conferring protection against oxygen-dependent DNA damage in P. gingivalis.Construction and characterization of a sod::lacZ variant. In order to examine the regulation of sod expression, a sod::lacZ translational fusion strain was constructed (Fig. 3). A single crossover event resulting in a P. gingivalis sod::lacZ genotype was confirmed by Southern blot hybridization with DNA probes derived from the sod and lacZ genes (data not shown). Furthermore, an intact copy of the sod gene was generated in CAL2 (sod::lacZ), as suggested by Southern blot analysis and subsequently confirmed by normal aerotolerance (data not shown). To our knowledge, this was the first reported demonstration of the utilization of the lacZ gene as a reporter gene in P. gingivalis (32). Subsequently, lacZ reporter constructs for other P. gingivalis genes have been reported (29, 64).
|
-galactosidase activity,
confirmed previously reported direct SOD activity measurements in
P. gingivalis under similar culture conditions
(3). Specifically, a twofold-greater induction of SOD
expression (measured at mid-log phase) was demonstrated when CAL2 was
cultured aerobically relative to when it was cultured anaerobically
(Fig. 4). In addition, sod expression at 45°C was significantly elevated relative to that at
37°C, as previously suggested by Northern blot analysis
(5). The combination of aerobic conditions with increased
temperatures produced an additive effect on
sod::lacZ expression.
|
-galactosidase
activity compared to mid-log-phase cultures and were invariably
unresponsive to known inducing conditions. Northern blot analysis (data
not shown) confirmed growth-dependent expression of the sod
gene. Therefore, all subsequent comparisons of effects on
sod expression were determined with the mid-log-phase cells.
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sod transcription initiation.
Since the regulation
of sod expression appears to occur at the transcriptional
level (5), it was of interest to attempt to identify
potential regulatory regions upstream of the sod gene. Therefore, the transcription start site of the sod gene was
determined to be 315 bp upstream of the sod start codon
(Fig. 7) and to be within an
uncharacterized upstream ORF, ORF2 (Fig. 1). There were no obvious
consensus 10 and 35 sequences when the sequence was compared to
previously suggested promoter region sequences for other P. gingivalis genes (29). The adenosine 315 bp upstream of
the start codon appears to be the major transcription start site for
sod, which would led to a transcript of approximately 0.9 kb. This was the size observed for sod mRNA on Northern blot analysis (reference 5 and data not shown). The
guanosine immediately downstream of the A base may act as a secondary
start site. Reverse transcription-PCR results obtained by using primers
present in the putative transcript further substantiated these findings
(data not shown). No DNA-binding consensus regions for known SOD
regulatory proteins in other organisms could be identified upstream of
the sod gene. Specifically, a search for consensus sequences
for Fur (58), integration host factor (46), and
Sox (63) operators revealed no significant homology.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Periodontal disease is a multifactorial entity in which complex microbial interactions are profoundly significant. The aerotolerant P. gingivalis appear to be capable of countering and even modifying the host response through a variety of mechanisms (66). While the importance of these potential virulence factors is clearly related to the survival ability of these organisms, it is also essential to consider the conditions that these organisms encounter in their colonization of the host. In particular, transmission and initial colonization events may pose the most crucial oxidative stresses to anaerobic organisms. With this in mind, it was logical to propose that the SOD enzyme may play its most significant role in these early events.
Our studies have demonstrated that while the P. gingivalis SOD is relatively selective in its response to a variety of environmental stresses, it obviously mediates at least one extremely important property, that of aerotolerance. Given the unique ecological demands that the oral cavity poses for anaerobic bacteria such as P. gingivalis, this aerotolerance may be as significant as any of the other potential virulence factors in this organism's armamentarium. This organism must first traverse the hostile oral cavity, an aerobic environment constantly bathed with saliva containing antimicrobial properties. Once overcoming this challenge, the organism must adhere to and colonize a complex biofilm, dental plaque. Although recent studies have detected P. gingivalis in supragingival plaque (65), itself an extremely competitive ecosystem, the organism is considered to be primarily a subgingival resident. Therefore, this organism must compete for a niche in the gingival crevice in the presence of host defense responses as well as in competition with other bacterial species.
SOD expression in P. gingivalis appears to be responsive to increased temperature, a key component of inflammation. This property appears to be distinct from the known heat shock response in this organism (35). Previous studies have suggested that increased temperatures may promote higher reactivity of oxygen radicals (9) and may induce gene expression through the alteration of DNA supercoiling (61).
The hydrogen peroxide biomodal killing pattern observed in E. coli (24) does not appear to be exhibited by P. gingivalis. In addition, whereas E. coli sodA sodB was more sensitive to mode-one killing by hydrogen peroxide (26), P. gingivalis CAL1 was no more sensitive than the parental organism. A pattern more suggestive of a linear response to hydrogen peroxide concentrations was observed in our study for P. gingivalis. Compared to E. coli, this organism was sensitive to lower levels of the peroxide, which may be expected from the obligate anaerobe.
A large and diverse range of microorganisms have evolved to utilize the long-lived mononuclear phagocytes as target cells to fulfill an obligate requirement for an intracellular environment in which to survive and replicate (49). While P. gingivalis certainly does not require an intracellular environment for survival, it is reasonable to consider whether this organism can evade prompt destruction after phagocytosis and possibly even persist intracellularly. During phagocytosis, ROS are confined to the phagocytic vacuole and serve as agents highly toxic to the internalized microbial agent. Some bacteria have developed means to resist the oxidative burst encountered within the phagolysosomes, and it has been suggested that SOD may protect Nocardia asteroides (7, 18) and Listeria monocytogenes and Shigella flexneri (42) from phagocytic killing as well. The SOD-deficient mutant, CAL1, did not appear to be more susceptible to killing by PMNs; this result is similar to that obtained in one study of E. coli deficient in the sodB gene (45). We have also found that extracellular ROS generated by pyrogallol killed the CAL1 mutant at rates similar to those for the parental organism. Therefore, these results indicate that the sod gene may not protect P. gingivalis from extracellular ROS. A previous study of P. gingivalis suggested that SOD is protective against killing by PMNs (4). However, in those experiments, purified P. gingivalis SOD was added to cultures, which allowed for the extracellular quenching of ROS, thus likely creating a nonnatural system for accurate assessment of this enzyme's function. However, it is possible that a periplasmic SOD similar to CuZnSODs, or even possibly nonspecific mechanisms, could play such a role in these organisms. No evidence for such an enzyme in these organisms has been reported, and our attempts to demonstrate such activity were inconclusive. The PMN is essentially a suicide cell, releasing an extraordinary oxidative burst that may override the antioxidant abilities of the cytoplasmic SOD in P. gingivalis, as suggested for other organisms (53). However, it is also possible that the SOD may protect the organism against oxidative killing by other phagocytes such as macrophages.
In addition, recent studies have demonstrated this organism's ability to invade, persist, and even replicate within certain host cell lines in vitro (31, 52). In a gingival epithelial cell culture, this organism was capable of intracellular replication and persisted within these cells over an 8-day period. It was found in the cytoplasm and was not confined by a membranous vacuole (34). It is reasonable to speculate that SOD may play a role in such intracellular survival.
Protection against oxygen-dependent DNA damage appears to be an important property of SOD in many organisms (25, 26). Indeed, a 6.8-fold-higher rate of spontaneous mutation to rifampicin resistance was observed in the sod mutant. P. gingivalis appears to have only a single sod gene, compared with the three found in E. coli. Two of these SODs in E. coli are found in the cytoplasm, and previous studies have demonstrated that MnSOD is highly protective against oxygen-dependent DNA damage, whereas the other, FeSOD, appears to confer modest protection at best (relative mutation rates of 8.7 and 0.9, respectively) (16). However, deletion of the two cytoplasmic-SOD genes resulted in a relative mutation rate of 41 compared to that for the wild-type strain. It was suggested that the greater protection provided by MnSOD in the sodB mutant was directly related to its inducibility. The observations that P. gingivalis contains only a single sod gene and that the CAL1 mutant exhibited a relatively high mutation rate compared to the wild type strongly suggest a critical role for SOD in protection against oxygen-dependent DNA damage in this periodontopathogenic bacterium.
In this study, we examined the regulation of expression of the sod gene in P. gingivalis. Although not well characterized in most organisms, the regulation of this gene relative to stress responses has received much attention in E. coli. For example, whereas the activity of FeSOD is similar under almost all growth conditions, the activity of MnSOD is modulated by oxidative environments both transcriptionally and posttranslationally in a metal-dependent fashion (47). Six global effectors of transcription are presently known to affect MnSOD expression (13). Homology searches for other superoxide stress-inducible genes and their corresponding transcriptional regulators in well-studied prokaryotes by using the P. gingivalis genome sequence (TIGR) did not yield any significant homologies. Interestingly, a similar search for genes involved in the hydrogen peroxide stress response, including the transcriptional regulator oxyR, did yield potential homologues, and we are currently investigating these findings. The possibility that the hydrogen peroxide stress response elements are present in this organism remains to be confirmed. However, if this indeed was the case, it would be of considerable interest, since P. gingivalis appears to be much more sensitive to hydrogen peroxide than to superoxide relative to other organisms studied to date. Furthermore, while CAL1 is highly sensitive to aerobiosis, it demonstrates a modest tolerance to exogenous ROS, equivalent to that of the parental organism. It is likely that nonspecific superoxide-protective elements exist in this organism and in some way account for these apparently selective protective qualities.
For many years, the CuZnSOD has been described as being present only in eukaryotes. However, at least 12 prokaryotic CuZnSOD gene sequences (designated sodC) have now been identified (10, 28, 30, 48, 57). Most of these organisms are animal pathogens, and many have host tissue invasion capabilities. CuZnSOD appears to be active in the periplasmic space, as opposed to the cytosol-restricted FeMnSOD, and it has been suggested that it may confer protection against extracellular superoxides such as those produced by activated neutrophils and macrophages. Preliminary attempts to identify the sodC gene in P. gingivalis by PCR methods or to identify its protein product by use of activity gels have been unsuccessful in our laboratory, and a BLAST search (1) of the unfinished genome failed to identify a potential homologue. This may further suggest a superoxide-protective role by nonspecific processes not yet identified.
In conclusion, we have found that SOD expression is dependent upon specific environmental conditions, including oxygen, increased temperature, and alkaline pH. It should be noted that these results are dependent upon the potential limitations of a translational fusion reporter system. However, in this study, results appeared to correspond well with Northern blot analyses of the wild-type organism under similar culture conditions. We have also confirmed that SOD indeed is crucial to the survival of P. gingivalis in aerobic environments as well as under conditions created by specific ROS. However, this enzyme does not appear to protect the organism against human neutrophils and exogenously generated superoxide. By conferring aerotolerance, this enzyme may be essential for colonization and infection in the oral cavity.
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ACKNOWLEDGMENTS |
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We thank M. Wilson for guidance and assistance with the PMN bactericidal assay and for providing the human hypogammaglobulinemic serum, R. Genco for providing the rabbit anti-P. gingivalis 2561 serum, and P. Bronson for assistance in the purification of immunoglobulin G.
This work was supported in part by NIH grants DE08293 and DE00158 and a Veterans Administration Dental Research Postdoctoral Fellowship.
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FOOTNOTES |
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* Corresponding author. Mailing address: Dept. of Oral Biology, State University of New York, 3435 Main St., Buffalo, NY 14214. Phone: (716) 829-2068. Fax: (716) 829-3942. E-mail: Kuramits{at}acsu.buffalo.edu.
Editor: J. R. McGhee
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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|---|
| 1. |
Altschul, S.,
T. Madden,
A. Schaffer,
J. Zhang,
W. Miller, and D. Lipman.
1997.
Gapped BLAST and PSI-BLAST: a new generation of protein database search programs.
Nucleic Acids Res.
25:3389-3402 |
| 2. | Amano, A., H. Tamagawa, S. Shizukuishi, and A. Tsunemitsu. 1986. Superoxide dismutase, catalase and peroxidases in oral anaerobic bacteria. J. Osaka Univ. Dent. Sch. 26:187-192[Medline]. |
| 3. |
Amano, A.,
S. Shizukuishi,
H. Tamagawa,
K. Iwakura,
S. Tsunasawa, and A. Tsunemitsu.
1990.
Characterization of superoxide dismutases purified from either anaerobically maintained or aerated Bacteroides gingivalis.
J. Bacteriol.
172:1457-1463 |
| 4. |
Amano, A.,
T. Ishimoto,
H. Tamagawa, and S. Shizukuishi.
1992.
Role of superoxide dismutase in resistance of Porphyromonas gingivalis to killing by polymorphonuclear leukocytes.
Infect. Immun.
60:712-714 |
| 5. |
Amano, A.,
A. Sharma,
H. Sojar,
H. Kuramitsu, and R. Genco.
1994.
Effects of temperature stress on expression of fimbriae and superoxide dismutase by Porphyromonas gingivalis.
Infect. Immun.
62:4682-4685 |
| 6. | Barua, P., D. Dyer, and M. Neiders. 1990. Effect of iron limitation on Bacteroides gingivalis. Oral Microbiol. Immunol. 5:263-268[Medline]. |
| 7. |
Beaman, L., and B. Beaman.
1990.
Monoclonal antibodies demonstrate that superoxide dismutase contributes to protection of Nocardia asteroides within the intact host.
Infect. Immun.
58:3122-3128 |
| 8. | Beauchamp, C., and I. Fridovich. 1971. Superoxide dismutase: improved assays and an assay applicable to polyacrylamide gels. Anal. Biochem. 44:276-287[Medline]. |
| 9. |
Benov, L., and I. Fridovich.
1995.
Superoxide dismutase protects against aerobic heat shock in Escherichia coli.
J. Bacteriol.
177:3344-3346 |
| 10. | Canvin, J., P. Langford, K. Wilks, and J. Kroll. 1996. Identification of sodC encoding periplasmic [Cu,Zn] superoxide dismutase in Salmonella. FEMS Microbiol. Lett. 136:215-220[Medline]. |
| 11. |
Choi, J.,
N. Takahashi,
T. Kato, and H. Kuramitsu.
1991.
Isolation, expression, and nucleotide sequence of the sod gene from Porphyromonas gingivalis.
Infect. Immun.
59:1564-1566 |
| 12. | Cohen, M., B. Britigan, Y. Chai, S. Pou, T. Roeder, and G. Rosen. 1991. Phagocyte-derived free radicals stimulated by ingestion of iron-rich Staphylococcus aureus: a spin-trapping study. J. Infect. Dis. 163:819-824[Medline]. |
| 13. |
Compan, I., and D. Touati.
1993.
Interaction of six global transcription regulators in expression of manganese superoxide dismutase in Escherichia coli K-12.
J. Bacteriol.
175:1687-1696 |
| 14. |
Cutler, C.,
J. Kalmar, and R. Arnold.
1991.
Phagocytosis of virulent Porphyromonas gingivalis by human polymorphonuclear leukocytes requires specific immunoglobulin G.
Infect. Immun.
59:2097-2104 |
| 15. |
Cutler, C.,
J. Kalmar, and R. Arnold.
1991.
Antibody-dependent alternate pathway of complement activation in opsonophagocytosis of Porphyromonas gingivalis.
Infect. Immun.
59:2105-2109 |
| 16. |
Farr, S.,
R. D'Ari, and D. Touati.
1986.
Oxygen-dependent mutagenesis in Escherichia coli lacking superoxide dismutase.
Proc. Natl. Acad. Sci. USA
83:8268-8272 |
| 17. |
Farr, S., and T. Kogoma.
1991.
Oxidative stress responses in Escherichia coli and Salmonella typhimurium.
Microbiol. Rev.
55:561-585 |
| 18. | Filice, G. 1983. Resistance of Nocardia asteroides to oxygen dependent killing by neutrophils. J. Infect. Dis. 148:861-867[Medline]. |
| 19. | Fletcher, H., H. Schenkein, R. Morgan, K. Bailey, C. Berry, and F. Macrina. 1995. Virulence of a Porphyromonas gingivalis W83 mutant defective in the prtH gene. Infect. Immun. 63:1521-1528[Abstract]. |
| 20. |
Franzon, V.,
J. Arondel, and P. Sansonetti.
1990.
Contribution of superoxide dismutase and catalase activities to Shigella flexneri pathogenesis.
Infect. Immun.
58:529-535 |
| 21. |
Genco, C.,
B. Odusanya, and G. Brown.
1994.
Binding and accumulation of hemin in Porphyromonas gingivalis are induced by hemin.
Infect. Immun.
62:2885-2892 |
| 22. | Hogg, N., V. Darley-Usmar, M. Wilson, and S. Moncada. 1992. Production of hydroxyl radicals from the simultaneous generation of superoxide and nitric oxide. Biochem. J. 281:419-424. |
| 23. |
Holt, S., and T. Bramanti.
1991.
Factors in virulence expression and their role in periodontal disease pathogenesis.
Crit. Rev. Oral Biol. Med.
2:177-281 |
| 24. |
Imlay, J., and S. Linn.
1986.
Bimodal pattern of killing of DNA-repair-defective or anoxically grown Escherichia coli by hydrogen peroxide.
J. Bacteriol.
166:519-527 |
| 25. |
Imlay, J.,
S. Chin, and S. Linn.
1988.
Toxic DNA damage by hydrogen peroxide through the Fenton reaction in vivo and in vitro.
Science
240:640-642 |
| 26. |
Imlay, J., and S. Linn.
1988.
DNA damage and oxygen radical toxicity.
Science
240:1302-1309 |
| 27. |
Imlay, J., and I. Fridovich.
1992.
Suppression of oxidative envelope damage by pseudoreversion of a superoxide dismutase-deficient mutant of Escherichia coli.
J. Bacteriol.
174:953-961 |
| 28. |
Imlay, K., and J. Imlay.
1996.
Cloning and analysis of sodC, encoding the copper-zinc superoxide dismutase of Escherichia coli.
J. Bacteriol.
178:2564-2571 |
| 29. |
Karunakaran, T.,
T. Madden, and H. Kuramitsu.
1997.
Isolation and characterization of a hemin-regulated gene, hemR, from Porphyromonas gingivalis.
J. Bacteriol.
179:1898-1908 |
| 30. |
Kroll, J.,
P. Langford, and B. Loynds.
1995.
Bacterial [Cu,Zn]-superoxide dismutase: phylogenetically distinct from the eukaryotic enzyme, and not so rare after all!
Microbiology
141:2271-2279 |
| 31. | Lamont, R., A. Chan, C. Belton, K. Izutsu, D. Vasel, and A. Weinberg. 1995. Porphyromonas gingivalis invasion of gingival epithelial cells. Infect. Immun. 63:3878-3885[Abstract]. |
| 32. | Lynch, M., and H. Kuramitsu. 1997. Study of superoxide dismutase in Porphyromonas gingivalis 381. J. Dent. Res. 76:abstract 320. |
| 33. |
Lynch, R., and I. Fridovich.
1978.
Permeation of the erythrocyte stroma by superoxide radical.
J. Biol. Chem.
253:4697-4699 |
| 34. | Madianos, P., P. Papapanou, U. Nannmark, G. Dahlen, and J. Sandros. 1996. Porphyromonas gingivalis FDC381 multiplies and persists within human oral epithelial cells in vitro. Infect. Immun. 64:660-664[Abstract]. |
| 35. | Maeda, H., M. Miyamoto, H. Hongyo, A. Nagai, H. Kurihara, and Y. Murayama. 1994. Heat shock protein 60 (GroEL) from Porphyromonas gingivalis: molecular cloning and sequence analysis of its gene and purification of the recombinant protein. FEMS Microbiol. Lett. 119:129-136[Medline]. |
| 36. | Marklund, S., and G. Marklund. 1974. Involvement of the superoxide anion radical in the autoxidation of pyrogallol and a convenient assay for superoxide dismutase. Eur. J. Biochem. 47:469-474[Medline]. |
| 37. |
Marsh, P.
1994.
Microbial ecology of dental plaque and its significance in health and disease.
Adv. Dent. Res.
8:263-271 |
| 38. |
McCord, J., and I. Fridovich.
1969.
Superoxide dismutase. An enzymatic function for erythrocuprein (hemocuprein).
J. Biol. Chem.
257:13977-13980 |
| 39. |
Meier, B.,
A. Sehn,
C. Michel, and M. Saran.
1994.
Reactions of hydrogen peroxide with superoxide dismutase from Propionibacterium shermanii an enzyme which is equally active with iron or manganeseare independent of the prosthetic metal.
Arch. Biochem. Biophys.
313:296-303[Medline].
|
| 40. |
Meyer, R., and J. Shapiro.
1980.
Genetic organization of the broad-host-range IncP-1 plasmid R751.
J. Bacteriol.
143:1362-1373 |
| 41. | Miller, J. 1972. Experiments in molecular genetics. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y. |
| 42. | Miller, R., and B. Britigan. 1997. Role of oxidants in microbial pathophysiology. Clin. Microbiol. Rev. 10:1-18[Abstract]. |
| 43. |
Nakayama, K.
1994.
Rapid viability loss on exposure to air in a superoxide dismutase-deficient mutant of Porphyromonas gingivalis.
J. Bacteriol.
176:1939-1943 |
| 44. |
Okamoto, K.,
K. Nakayama,
T. Kadowaki,
N. Abe,
D. Ratnayake, and K. Yamamoto.
1998.
Involvement of a lysine-specific cysteine proteinase in hemoglobin absorption and heme accumulation by Porphyromonas gingivalis.
J. Biol. Chem.
273:21225-21231 |
| 45. |
Papp-Szabo, E.,
C. Sutherland, and P. Josephy.
1993.
Superoxide dismutase and the resistance of Escherichia coli to phagocytic killing by human neutrophils.
Infect. Immun.
61:1442-1446 |
| 46. | Presutti, D., and H. Hassan. 1995. Binding of integration host factor (IHF) to the Escherichia coli sodA gene and its role in the regulation of a sodA-lacZ fusion gene. Mol. Gen. Genet. 246:228-235[Medline]. |
| 47. |
Privalle, C., and I. Fridovich.
1992.
Transcriptional and maturational effects of manganese and iron on the biosynthesis of manganese-superoxide dismutase in Escherichia coli.
J. Biol. Chem.
267:9140-9145 |
| 48. | Puget, K., and A. Michelson. 1974. Isolation of a new copper-containing superoxide dismutase bacteriocuprein. Biochem. Biophys. Res. Comm. 58:830-838[Medline]. |
| 49. | Reiner, N. 1994. Altered cell signaling and mononuclear phagocyte deactivation during intracellular infection. Immun. Today 15:374-381. |
| 50. | Ryan, C., and I. Kleinberg. 1995. Bacteria in human mouths involved in the production and utilization of hydrogen peroxide. Arch. Oral Biol. 40:753-763[Medline]. |
| 51. |
Sadowsky, A.,
J. Wilson,
H. Steinman, and H. Shuman.
1994.
The iron superoxide dismutase of Legionella pneumophila is essential for viability.
J. Bacteriol.
176:3790-3799 |
| 52. | Sandros, J., P. Papapanou, U. Nannmark, and G. Dahlen. 1994. Porphyromonas gingivalis invades human pocket epithelium in vitro. J. Periodontal Res. 29:62-69[Medline]. |
| 53. |
Schwartz, C.,
J. Krall,
L. Norton,
K. McKay,
D. Kay, and R. Lynch.
1983.
Catalase and superoxide dismutase in Escherichia coli.
J. Biol. Chem.
258:6277-6281 |
| 54. |
Scott, M.,
S. Meshnick, and J. Eaton.
1987.
Superoxide dismutase-rich bacteria.
J. Biol. Chem.
262:3640-3645 |
| 55. |
Shapira, S.,
J. Chou,
F. Richard, and M. Casadaban.
1983.
New versatile plasmid vectors for expression of hybrid proteins coded by a cloned gene fused to lacZ gene sequences encoding enzymatically active carboxyl-terminal portions of -galactosidase.
Gene
25:71-82[Medline].
|
| 56. | Shibata, Y., and H. Kuramitsu. 1996. Isolation and preliminary characterization of the Streptococcus mutans rpsJ gene. Oral Microbiol. Immunol. 11:407-411[Medline]. |
| 57. |
Steinman, H.
1987.
Bacteriocuprein superoxide dismutase of Photobacterium leiognathi.
J. Biol. Chem.
262:1882-1887 |
| 58. | Stojiljkovic, I., A. Baumler, and K. Hantke. 1994. Fur regulon in Gram-negative bacteria. J. Mol. Biol. 236:531-545[Medline]. |
| 59. | Tanner, A., C. Haffer, G. Bratthall, R. Visconti, and S. Socransky. 1979. A study of the bacteria associated with advancing periodontitis in man. J. Clin. Periodontol. 6:278-307[Medline]. |
| 60. | Tokuda, M., M. Duncan, M.-I. Cho, and H. Kuramitsu. 1996. Role of Porphyromonas gingivalis protease activity in colonization of oral surfaces. Infect. Immun. 64:4067-4073[Abstract]. |
| 61. | Tse-Dinh, Y., H. Qi, and R. Menzel. 1997. DNA supercoiling and bacterial adaptation: thermotolerance and thermoresistance. Trends Microbiol. 5:323-326[Medline]. |
| 62. | Wilson, M., P. Bronson, and R. Hamilton. 1995. Immunoglobulin G2 antibodies promote neutrophil killing of Actinobacillus actinomycetemcomitans. Infect. Immun. 63:1070-1075[Abstract]. |
| 63. |
Wu, J., and B. Weiss.
1991.
Two divergently transcribed genes, soxR and soxS, control a superoxide response regulon of Escherichia coli.
J. Bacteriol.
173:2864-2871 |
| 64. | Xie, H., S. Cai, and R. Lamont. 1997. Environmental regulation of fimbrial gene expression in Porphyromonas gingivalis. Infect. Immun. 65:2265-2271[Abstract]. |
| 65. | Ximenez-Fyvie, L., A. Haffajee, and S. Socransky. 1998. Comparison of the microbial composition of supra- and subgingival plaque. J. Dent. Res. 77:abstract 150. |
| 66. |
Yoneda, M.,
K. Maeda, and M. Aono.
1990.
Suppression of bactericidal activity of human polymorphonuclear leukocytes by Bacteroides gingivalis.
Infect. Immun.
58:406-411 |
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